HUE028363T2 - Anti-ICAM antibody inducing apoptosis. - Google Patents

Anti-ICAM antibody inducing apoptosis. Download PDF

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HUE028363T2
HUE028363T2 HUE06829616A HUE06829616A HUE028363T2 HU E028363 T2 HUE028363 T2 HU E028363T2 HU E06829616 A HUE06829616 A HU E06829616A HU E06829616 A HUE06829616 A HU E06829616A HU E028363 T2 HUE028363 T2 HU E028363T2
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Bjoern Frendeus
Roland Carlsson
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Bioinvent Int Ab
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Abstract

The invention provides binding molecules, including antibody molecules which selectively bind to a cell surface antigen of a target cell, and wherein the binding molecules, on binding the cell surface antigen, induce apoptosis of the target cell. There is also provided methods of and pharmaceutical compositions for apoptosis induction and uses thereof.

Description

Description [0001] The invention relates to molecules involved in apoptosis induction, methods and pharmaceutical compositions for apoptosis induction and uses thereof.
[0002] Antibodies have recently become the protein therapeutics of choice for targeting cancer but also for treating other indications (Brekke et al. Nat Rev Drug Discov 2003;2:52-62). The advent of antibody engineering has provided the tools to generate human antibodies from synthetic phage libraries, displaying decreased immunogenicity and enhanced specificity and affinity due to their human nature and greater diversity (Weiner et al. Nat Biotechnol 2005;23:556-7). Naïve libraries are particularly attractive, as they may be used for isolation of antibodies for any specificity, including self-antigens (Griffiths et al. Embo J 1993;12:725-34), independent of immunizations and reconstruction of new libraries. Cell surface receptors constitute by far the most successful group of antigens targeted by contemporary therapeutic drugs, including small molecule inhibitors and antibodies. Of particular interest are cell surface receptors that are uniquely expressed or that display an increased expression level on a target cell and are additionally capable of relaying death or survival signals to the cell. Such differentially expressed receptors with intrinsic signalling properties enable antibody-based targeting of microbial infected, transformed, or otherwise malfunctioning cells.
[0003] For treatment of tumours, antibodies that have the ability to induce apoptosis in a target tumour cell whilst sparing normal tissue are of particular interest. Several such antibodies are in use, have been registered with the US Food and Drug Administration (FDA) and provide alternatives to conventional cancer treatments e.g. for lymphoma (rituximab targeting CD20) or for breast cancer (trastuzumab or cetuximab targeting Her-2 and EGFR respectively).
[0004] There are also other antibodies with apoptosis inducing efFects currently in clinical development. However, even if these antibodies demonstrate beneficial effects in patients or in animal tests an unmet clinical need still exists.
[0005] Anti-idiotypic immunoglobulin targeting of B cell tumours was the first monoclonal antibody therapy conducted in man (Miller et al. N Engl J Med 1982;306:517-22.). Destruction of tumour cells by such means of passive antibody administration (Riechmann et al. Nature 1988;332:323-7.), or active vaccination with the patients own tumour immunoglobulin protein (Kwak et al. N Engl J Med 1992;327:1209-15.), has since been demonstrated to confer tumour regression or tumour dormancy in patients with different kinds of B cell malignancies. A more recent report describes the generation of fully human anti-idiotype antibodies using transgenic mice deficient in mouse antibody production and expressing selected human antibody chain loci (Suarez et al. Mol Immunol 2004;41:519-26.).
[0006] In the present invention a competition biopanning method has been used, where target cell antigen in the form of whole cells, and excess subtractor cell antigen in the form of membrane vesicles, are exposed at the same time to the naive n-CoDeR® antibody phage library (WO 2004/023140; Soderlind et al. Nat Biotechnol 2000;18:852-6.), to retrieve and subsequently test antibody fragments with excellent selectivity for B lymphoma target cells. Furthermore, functionality in the selected binding molecules was demonstrated by the ability of the antibodies tested to induce apoptosis in target but not in non-target cells.
[0007] Antibody specificities identified include HLA-DR/DP (the B1 antibody of the invention) and surface IgM (the C11 antibody of the invention), as well as ICAM-1 (the B11 antibody of the invention), an adhesion molecule not previously associated with apoptosis induction. Isolated antibodies had affinities in the subnanomolar to nanomolar range, directly making them possible choices for targeted antibody therapy.
Summary of the Invention [0008] In a first aspect of the invention there is provided a method of inducing apoptosis in a target cell comprising the steps: a. providing one or more target cells displaying the cell surface antigen, ICAM-1; b. providing one or more binding molecules which selectively binds to cell surface ICAM-1 and, on binding ICAM-1, induces apoptosis of the target cell; c. exposing the target cells of (a) to the binding molecules of (b) to induce apoptosis in the target cells.
[0009] Wherein the binding molecule is an antibody molecule having variable regions having the sequences of figures 10.
[0010] In the disclosure is provided a method of inducing apoptosis in a target cell comprising the steps: a. providing one or more target cells displaying the cell surface antigen, HLA-DR/DP and/or surface IgM; b. providing one or more antibody molecules which selectively binds to cell surface HLA-DR/DP and/or surface IgM and, on binding HLA-DR/DP and/or surface IgM, inducing apoptosis of the target cell; c. exposing the target cells of (a) to the antibody molecules of (b) to induce apoptosis in the target cells.
[0011] In a further aspect of the invention there is provided a binding molecule which selectively binds to cell surface ICAM-1 and, on binding ICAM-1, induces apoptosis of the target cell and is a human antibody having the variable regions having the sequences of figure 10.
[0012] ICAM-1 is also designated CD54, but for the purpose of this application ICAM-1 will be used.
[0013] Binding molecules may be derived from antibodies and based on the antibody scaffold [Clackson T et al., Nature. 1991 Aug 15;352(6336):624-8, Marks JD et al., J Mol Biol. 1991 Dec 5;222(3):581-97] that has been used extensively in many libraries, but binding molecules may also be derived form other molecular scaffolds such as the fibronectin scaffold [Weng S et al., Proteomics. 2002 Jan;2(1 ):48-57] and the protein A scaffold [Nord K, et al.,Nat Biotechnol 1997 Aug;15(8):772-7, Hogbom M et al., Proc Natal Acad Sei USA. 2003 Mar 18;100(6):3191-6], Each of these scaffolds may have their advantages depending on application, and the antibody scaffold, as one example, may be used advantageously for creating variability indistinguishable from natural variability.
[0014] The basic structure of the antibody, the most commonly used scaffold, is very well understood. In principle, a framework structure comprising beta strands ordered into two sheets present a set of variable loops, the so called Complementary Determining Regions (CDRs) that have the capacity to bind to antigen molecules. Although antibodies may vary in the scaffold structure the most extensive variability is seen in the CDRs. The great variability in-between antibodies, is the basis for their ability to interact, in a specific manner, with in principle all types of molecular structures. Due to this capacity, antibodies have been used extensively for generation of specific binders with applicability within research, diagnosis/prognosis of disease and as therapeutic agents specific for defined target structures [Borrebaeck CA and Carlsson R, Curr Opin Pharmacol. 2001 Aug; 1(4):404-8].
[0015] Other, non-antibody binding molecules are those having scaffold structures with a high degree of stability yet allowing variability to be introduced at certain positions. An example of another binding molecule is a fibronectin domain and a 58 amino acids large protein A domain which tolerate variability. There are also other molecular folds that allow some degree of variation. Such examples include major histocompatibility complex (MHC) class I and II molecules and recently a novel class of molecules the so called defensins have been identified to be similar in basic structure while still harbouring extensive sequence variability in-between the gene family members indicating that they are suitable as scaffolds for harbouring molecular diversity. In addition, natural ligand(s) e.g. LFA-1 in the case of ICAM-1 as a target molecule, or recombinant variants of them, may constitute specific binding molecules able to induce apoptosis in target cells.
[0016] Furthermore, the binding molecule may be any molecule selectively binding cell surface ICAM-1 of a target cell and, on binding, inducing apoptosis of the target cell.
[0017] The present screening retrieved an antibody (B11) specific for ICAM-1 - a receptor not previously associated with apoptosis and not attributed intrinsic negative signalling properties in cells.
[0018] The identification of ICAM-1 as an apoptosis-inducing molecule was a direct result of the screening being designed to isolate specificities for all surface receptors differentially expressed between target and non-target cells, irrespective of and without prior knowledge of their respective identity. ICAM-1-induced cell death has been verified as an active apoptotic process that involved mitochondrial membrane depolarisation. Mitochondrial membrane depolarisation has been previously described for both caspase dependent and caspase independent apoptosis (Nagy et al. J Mol Med 2003;81:757-65.).
[0019] The present findings further show that the epitope bound by the B11 antibody is expressed in B lymphoma tissue of different origin, and is up regulated in certain B lymphoma cells compared to resting peripheral blood leukocytes. Importantly, in addition to B lymphoma cells also carcinoma cells expressing ICAM-1 underwent apoptosis when subjected to the ICAM-1 specific B11 antibody in vitro (see Example 6).
[0020] Previous studies have demonstrated restricted expression of ICAM-1 on normal human tissues (Smith et al. J Clin Pathol 1990;43:893-900.). ICAM-1 is involved in cell to cell adhesion and plays an important role in immune responses and inflammation through binding to its receptor LFA-1. Antibodies directed to ICAM-1 have been used to interfere with pathological immune responses and inflammation. In vivo administration of a murine anti-ICAM-1 mAb in cymologous monkeys (Cosimi étal. J Immunol 1990;144:4604-12.), or use in clinical trials in human patients with rheumatoid arthritis or patients receiving kidney transplants has also revealed no overt toxicity (Kavanaugh et al. Arthritis Rheum 1994;37:992-9; Haug et al. Transplantation 1993;55:766-72.).
[0021] The novel finding that ICAM-1 targeting can lead to apoptosis demonstrates the possibility to use ICAM-1 specific binding molecules, such as antibodies for treatment of cancers of different origins provided that they express the antigen.
[0022] Based on their expression of ICAM-1 cancer types that may potentially be treated with an apoptosis inducing anti-ICAM-1 antibody such as B11 include: B lymphoma, myeloma (Huang et al. (1993) Hybridoma 12 p661-75; Huang et al., (1995) Cancer Res 55 p610-6; Smallshaw et al., (2004) J lmmunother27 p419-24), gastric cancer (Maruo et al., (2002) Int J Cancer 100 p486-90), breast cancer (Rosette et al., (2005) Carcinogenesis 26 p943-50), liver cancer (Sun etal.,(1999) J Cancer Res Clin Oncol 125 p28-34), lung cancer (Grothey et al., (1998) Br J Cancer77 p801-7 ), melanoma (Wang et al., (2005) Int J Cancer 27 p419-24), bladder cancer (Roche et al., (2003) Thromb Haemost 89 1089-97) and prostate cancer (Aalinkeel et al., (2004) Cancer Res 64 p5311-21). Expression of ICAM-1 has also been identified in tumour metastasis as demonstrated by (Maruo et al., 2002), (Rosette et al., 2005), (Sun et al., 1999), (Grothey et al., 1998), (Aalinkeel et al., 2004) pointing to the possibility to intervene in metastasis processes using an ICAM-1 specific antibody.
[0023] In a further disclosure the cell surface antigen is HLA-DR/DP.
[0024] HLA-DR/DP is normally present on, for example, B cells and can be found up-regulated on B lymphoma cells.
[0025] To date, three different HLA-DR specific monoclonal antibodies have entered clinical phase trials. The most recent addition of which is the fully human lgG4 1D09C3, which was isolated from a similarly sized naive phage library compared to n-CoDeR®, but using solid phase panning on purified antigen (Nagy et al. Nat Med 2002;8:801-7.).
[0026] A novel human antibody (B1 ) directed against HLA-DR/DP that rapidly and with high potency induces apoptosis in a multitude of B-lymphoma cell lines has been identified thereby demonstrating HLA-DR/DP is linked to the induction of apoptosis in a target cell.
[0027] The B1 antibody bound a multitude of B lymphoma cell lines of different origin (see Example 1 and Table 1) and was shown to induce apoptosis in HLA-DR/DP antigen expressing cells. Furthermore, the B1 antibody showed a higher potency than Rituximab when tested on the Raji B lymphoma cell line. This was particularly evident, when the lgG4 format of the B1 antibody was used (Figure 8).
[0028] From the data obtained, this antibody has suitable characteristics for treatment of HLA-DR/DP expressing B lymphoma cells. In addition, similar to the targeting of Rheumatoid Arthritis and SLE by Rituximab, the B1 antibody may prove efficacious in eliminating activated B cells in disorders where HLA-DR/DP expressing B cells are detrimental.
[0029] In a yet further disclosure the cell surface antigen is surface IgM.
[0030] IgM in its free form exists as a large pentameric structure, whose higher molecular weight tends to confine it within blood vessels.
[0031] Monomeric IgM can be found on the cell walls of B lymphocytes and functions as an antibody receptor for antigen recognition.
[0032] The C11 antibody, upon binding to surface IgM, expressed on B lymphoma cells, induces apoptosis in a rapid and efficient manner (see Example 1 and Table 1). In contrast to the idiotype specific anti-IgM antibodies previously used in the clinic for treatment of B lymphoma the C11 antibody bind to a non-polymorphic epitope expressed on B cells from different donors and is thus suitable for treatment of patients suffering from B lymphoma irrespective of B lymphoma idiotype.
[0033] Notably, the effector molecule e.g. the anti-IgM antibody could also be any type of specific binding molecule that causes apoptosis in IgM expressing cells of different idiotypes.
[0034] The kinetics of B1, B11 and C11 IgG induced apoptosis were fast, with maximal efficacy being observed already after 3 hours in some cell lines. Rapid effector function is important for therapeutic efficacy as this minimizes the risk for tumour evasion resulting from e.g. lack of expression of tumour antigen (Uyttenhove étal. J. Exp. Med. 1983;157:1040-52; Kennedy et al. Br J Haematol 2002;119:412-6) or epitope mutation (Weiner et al. J Immunol 1989;142:343-51 ; Bai et al. J. Clin. Invest. 2003;111:1487-96), and potentially limits treatment duration and side-effects (Robert et al. Lancet Oncol 2005;6:491-500.).
[0035] Preferably the target cell is an immune cell or epithelial cell and advantageously that immune cell is a B lymphocytes.
[0036] Conveniently the target cell is associated with a disease. Preferably the disease is selected from the group consisting of: cancer; autoimmune diseases including but not restricted to rheumatoid arthritis and SLE, acute and chronic inflammatory disorders, sepsis and infectious disease including but not restricted to HIV.
[0037] Advantageously, the disease is a cancer selected from lymphoma (leukaemia, myeloma), gastric cancer, breast cancer, liver cancer, lung cancer, melanoma, bladder cancer, chorioid cancer, pancreatic cancer, colon cancer and prostate cancer.
[0038] Conveniently, the antibody molecule is an IgG. The IgG may be any of lgG1, lgG2, lgG3 or lgG4, but preferably any of lgG1 and lgG4. The antibody molecule is preferably human.
[0039] Conveniently, the binding molecule or antibody molecule of the invention has the sequence of any one of variable region sequences of Figure 10 [0040] In one embodiment of the disclosure the binding molecule or antibody molecule has the variable region sequences of Figure 9 or functionally equivalent homologues thereof.
[0041] In a yet further embodiment of the disclosure, the binding molecule or antibody molecule has the variable region sequences of Figure 11 or functionally equivalent homologues thereof.
[0042] Conveniently the nucleic acid has the nucleotide sequence of any one of figures 9 to 11.
[0043] In a further aspect of the invention there is provided use of the antibody molecule of the invention in the diagnosis and/or treatment and/or prevention of a disease requiring the destruction of a target cell. There is also provided the use of the antibody molecule of the invention in the molecule of the invention in the manufacture of a medicament for the treatment and/or prevention of a disease requiring the destruction of a target cell.
[0044] Conveniently, the disease to be treated is selected from the group consisting of: cancer; autoimmune diseases including but not restricted to rheumatoid arthritis and SLE, acute and chronic inflammatory disorders, sepsis and infectious disease including but not restricted to HIV.
[0045] Advantageously the disease to be treated is cancer selected from lymphoma (leukaemia, myeloma), gastric cancer, breast cancer, liver cancer, lung cancer, melanoma, bladder cancer, chorioid cancer, pancreatic cancer, colon cancer and prostate cancer.
[0046] In one embodiment of the invention the binding molecule or antibody molecule binds specifically to ICAM-1 and/or has the sequence of figure 10 and is used in relation to the diseases listed above.
[0047] In a further embodiment of the disclosure the antibody molecule binds specifically to HLA-DR/DP and/or has the sequence of figure 9 and is used in relation to the diseases of lymphoma (leukaemia, myeloma), gastric cancer, breast cancer, liver cancer, lung cancer, melanoma, bladder cancer, chorioid cancer, pancreatic cancer, colon cancer and prostate cancer.
[0048] In a yet further embodiment of the disclosure the antibody molecule binds specifically to surface IgM and/or has the sequence of figure 11 and is used in relation to the diseases of lymphoma (leukaemia, myeloma), gastric cancer, breast cancer, liver cancer, lung cancer, melanoma, bladder cancer, chorioid cancer, pancreatic cancer, colon cancer and prostate cancer.
[0049] In a further aspect of the invention there is provided a pharmaceutical composition comprising the antibody molecule of the invention and a pharmaceutically acceptable carrier, excipient or diluent.
Meanings of terms used [0050] The term "antibody molecule" shall be taken to refer to any one of an antibody, an antibody fragment, or antibody derivative. It is intended to embrace wildtype antibodies, synthetic antibodies, recombinant antibodies or antibody hybrids, such as, but not limited to, a single-chain modified antibody molecule produced by phage-display of immunoglobulin light and/or heavy chain variable and/or constant regions, or other immunointeractive molecules capable of binding to an antigen in an immunoassay format that is known to those skilled in the art.
[0051] The term "antibody fragment" shall be taken to refer to any one of an antibody, an antibody fragment, or antibody derivative. It is intended to embrace wildtype antibodies (i.e. a molecule comprising four polypeptide chains), synthetic antibodies, recombinant antibodies or antibody hybrids, such as, but not limited to, a single-chain modified antibody molecule produced by phage-display of immunoglobulin light and/or heavy chain variable and/or constant regions, or other immunointeractive molecules capable of binding to an antigen in an immunoassay format that is known to those skilled in the art.
[0052] The term "antibody derivative" refers to any modified antibody molecule that is capable of binding to an antigen in an immunoassay format that is known to those skilled in the art, such as a fragment of an antibody (e.g. Fab or Fv fragment), ora modified antibody molecule that is modified by the addition of one or more amino acids or other molecules to facilitate coupling the antibodies to another peptide or polypeptide, to a large carrier protein or to a solid support (e.g. the amino acids tyrosine, lysine, glutamic acid, aspartic acid, cysteine and derivatives thereof, NH2-acetyl groups or COOH-terminal amido groups, amongst others).
[0053] The term "ScFv molecule" refers to any molecules wherein the VH and VL partner domains are linked via a flexible oligopeptide.
[0054] The terms "nucleotide sequence" or "nucleic acid" or "polynucleotide" or "oligonucleotide" are used interchangeably and refer to a heteropolymer of nucleotides or the sequence of these nucleotides. These phrases also refer to DNA or RNA of genomic or synthetic origin which may be single-stranded or doublestranded and may represent the sense or the antisense strand, to peptide nucleic acid (PNA) or to any DNA-like or RNA-like material. In the sequences herein A is adenine, C is cytosine, T is thymine, G is guanine and N is A, C, G or T (U). It is contemplated that where the polynucleotide is RNA, the T (thymine) in the sequences provided herein is substituted with U (uracil). Generally, nucleic acid segments provided by this invention may be assembled from fragments of the genome and short oligonucleotide linkers, or from a series of oligonucleotides, or from individual nucleotides, to provide a synthetic nucleic acid which is capable of being expressed in a recombinant transcriptional unit comprising regulatory elements derived from a microbial or viral operon, or a eukaryotic gene.
[0055] The terms "polypeptide" or "peptide" or "amino acid sequence" refer to an oligopeptide, peptide, polypeptide or protein sequence or fragment thereof and to naturally occurring or synthetic molecules. A polypeptide "fragment," "portion," or "segment" is a stretch of amino acid residues of at least about 5 amino acids, preferably at least about 7 amino acids, more preferably at least about 9 amino acids and most preferably at least about 17 or more amino acids. To be active, any polypeptide must have sufficient length to display biological and/or immunological activity.
[0056] The terms "purified" or "substantially purified" as used herein denotes that the indicated nucleic acid or polypeptide is present in the substantial absence of other biological macromolecules, e.g., polynucleotides, proteins, and the like. In one embodiment, the polynucleotide or polypeptide is purified such that it constitutes at least 95% by weight, more preferably at least 99% by weight, of the indicated biological macromolecules present (but water, buffers, and other small molecules, especially molecules having a molecular weight of less than 1000 daltons, can be present).
[0057] The term "isolated" as used herein refers to a nucleic acid or polypeptide separated from at least one other component (e.g., nucleic acid or polypeptide) present with the nucleic acid or polypeptide in its natural source. In one embodiment, the nucleic acid or polypeptide is found in the presence of (if anything) only a solvent, buffer, ion, or other component normally present in a solution of the same. The terms "isolated" and "purified" do not encompass nucleic acids or polypeptides present in their natural source.
[0058] The term "recombinant," when used herein to refer to a polypeptide or protein, means that a polypeptide or protein is derived from recombinant (e.g., microbial, insect, or mammalian) expression systems. "Microbial" refers to recombinant polypeptides or proteins made in bacterial or fungal (e.g., yeast) expression systems. As a product, "recombinant microbial" defines a polypeptide or protein essentially free of native endogenous substances and unaccompanied by associated native glycosylation. Polypeptides or proteins expressed in most bacterial cultures, e.g., Escherichia coli, will be free of glycosylation modifications; polypeptides or proteins expressed in yeast will have a glycosylation pattern in general different from those expressed in mammalian cells.
[0059] The terms "selective binding" and "binding selectivity" indicates that the variable regions of the antibodies of the invention recognise and bind polypeptides of the invention exclusively (i.e., able to distinguish the polypeptide of the invention from other similar polypeptides despite sequence identity, homology, or similarity found in the family of polypeptides), but may also interact with other proteins (for example, Staphylococcus aureus protein A or other antibodies in ELISA techniques) through interactions with sequences outside the variable region of the antibodies, and in particular, in the constant region of the molecule. Screening assays to determine binding selectivity of an antibody of the invention are well known and routinely practiced in the art. For a comprehensive discussion of such assays, see Harlow et al. (Eds), Antibodies A Laboratory Manual; Cold Spring Harbor Laboratory; Cold Spring Harbor, N.Y. (1988), Chapter 6. Antibodies that recognise and bind fragments of the polypeptides of the invention are also contemplated, provided that the antibodies are first and foremost selective for, as defined above, full-length polypeptides of the invention. As with antibodies that are selective for full length polypeptides of the invention, antibodies of the invention that recognise fragments are those which can distinguish polypeptides from the same family of polypeptides despite inherent sequence identity, homology, or similarity found in the family of proteins.
[0060] The term "binding affinity" includes the meaning of the strength of binding between an antibody molecule and an antigen.
[0061] By the term "immune cell" we mean any cell that is involved in a host immune or inflammatory response, including but not limited to B cells and T cells.
[0062] By the term "epithelial cell" we mean a cell of the epithelium. Epithelium is a tissue composed of a layer of cells. Epithelium can be found lining internal (e.g. endothelium, which lines the inside of blood vessels) or external (e.g. skin) free surfaces of the body.
[0063] The outermost layer of our skin is composed of squamous epithelial cells, as are the mucous membranes lining the inside of mouths and body cavities. Other epithelial cells line the insides of the lungs, the gastrointestinal tract, the reproductive and urinary tracts, and make up the exocrine and endocrine glands. Functions of epithelial cells include secretion, absorption and protection. Epithelial cells sit on a basal lamina.
Preferred Embodiments [0064] Examples embodying certain preferred aspects of the invention will now be described with reference to the following figures in which: -
Figure 1 - scFv isolated by differential whole cell/ cell membrane vesicle biopanning show high target cell specificity. scFv clones isolated by differential biopanning were expressed in E. coli TOP 10 cells and incubated with Ramos or Jurkat cells and (A) scFv clones expressed for primary screening or (B) seventy two randomly picked and reexpressed scFv clones. Bound scFv was detected with anti-His MAb, and Cy5-anti-mouse polyclonal Ab. Cell binding was detected in an FMAT Macroconfocal High Throughput Screening instrument. Cell binding is depicted as mean fluorescence intensity to target Ramos cells (Y axis) vs. non-target Jurkat cells (X-axis). (C) Binding of seven unique scFv clones to Ramos cells (filled bars) and Jurkat cells (open bars). A control scFv (ctrl) did not bind to any of the cells.
Figure 2. Apoptosis induction of anti-Ramos scFv.
Ramos B lymphoma cells were sequentially incubated with anti-Ramos scFv, anti-His mAb, and anti-mouse polyclonal Ab on ice (with intermittent washing to remove excess unbound antibody), and were incubated in a humidified atmosphere of 5 % C02 at 37 °C for 24 hours. Cells were then harvested and subjected to combined staining with Annexin V-AF488 (AV) and propidium iodide (PI). Cells were scored as viable (AV- PI-, filled circles Fig. 2C), early apoptotic (AV+ PI-, open triangles Fig. 2C), or late apoptotic/ necrotic (AV+ PI-s-, open diamonds Fig. 2C), based on differential positivity for AV and PI staining (defined by square gates in Fig. 2B). Results are presented by plotting (A) Forward Scatter (FSC-Height) against Side Scatter and (B) AV (FL-1) against PI (FL-3). The titratable effect of scFv B1 and F1 is also presented (C). The seven unique scFv clones were incubated with (D) Ramos or (E) Raji B lymphoma cells at 37 °Cfor 24 hours at various concentrations and the effect on apoptosis induction studied. Three scFv; B1, B11, and C11, show titratable activity towards both cell lines, whereas apoptosis inducing capability of scFv B10, C10, and G12 is restricted to Ramos B lymphoma cells.
Figure 3. Specificities of isolated antibodies include HLA-DR/DP, IgM, and ICAM-1. A) 50-600 X 106 Raji B lymphoma cells were lysed with the non-ionic detergent Triton X-100 at 0.5 % v/v and immunoprecipitated with 100 μg of the fully human lgG1 format of B1 (lane 1) and B11 (lane 2) antibody, followed by crosslinking with Protein A Sepharose. Ramos B lymphoma cell lysates, from 50 x 106 cells, were used for the precipitation of 20 μg C11 (lane 3). Antibody-specific bands were excised and subjected to tryptic digestion and analysed by MALDI-TOF. B) B1 IgG, B11 IgG, and C11 IgG binding to B lymphoma cells is specifically blocked by pre-incubation with anti-HLA-DR/DP, anti-ICAM-1 oranti-IgM antibodies, respectively.
To confirm the retrieved MALDI-TOF antigen identities of antibody clones B1, B11, and C11, blocking studies with commercially available antibodies was carried out and analyzed by flow cytometry. Cells were pre-blocked with 10-fold molar excess (compared to the human antibody) of species-matched blocking antibodies for 1 h, followed by the addition of any of the isolated human antibody clones. After 30 min, cells were washed and binding of human antibody to cells was detected by PE-conjugated goat anti-human IgG (Caltag Laboratories, Burlingame, CA, USA). The blocking antibodies used in the study were; for B1, mouse monoclonals anti-HLA DR (Sigma, clone HK14) or anti-CD40 (Beckton Dickinson, clone 5C3); for B11, rabbit polyclonals anti-ICAM-1 (Abeam, ab7815-250) oranti-CD22 (Abeam, ab25135-100); forC11, goat polyclonals anti-IgM (Zymed, South San Francisco, CA, USA, 62-7500) or anti-IgG (Zymed, 62-8400).
Figure 4. ICAM-1 is a B lymphoma associated cell surface receptor capable of mediating programmed cell death. A. 2 μg/ml of B11 or anti-FITC-8 (control) lgG1 was added to 4 x 105 CL-01 B lymphoma cells, incubated for2 h on ice, followed by addition of 10 μg/ml crosslinking secondary Fab’2 Goat anti-human Fc antibody. Cells were incubated at 37 °C for 6 h and the effect of the antibody incubation was determined by two independent apoptosis assays. Cells were stained either by AV/PI (upper panel), similarly as described above, or by incubation with 5 μg/mlofthe mitochondrial membrane depolarisation reagent JC-1 for 30 min atRT (lower panel). Induction of apoptosis is detectable by a decrease in the red (y-axis)/green (x-axis) fluorescence intensity ratio. (B) Histology section showing representative binding of B11 antibody to B lymphoma tissue. Cryo-preserved tissue obtained from a patient with Anaplastic Large Cell B Lymphoma was stained with B 11 or FITC-8 (control) scFv antibody. Antibody binding was detected with DAB (brown colour). Inset picture shows staining with control scFv. (C) CD45-PerCp-Cy5.5 mAb pre-labelled Ramos cells were mixed with donor-derived PBMCs and the different cell populations were stained with fluorochrome-conjugated CD-specific antibodies and Alexa Flour 647 Zenon pre-labelled B11 lgG1 or control FITC-8 lgG1. IgG B11 binding to the different cell populations was recorded in the FL4 channel.
Figure 5. Affinities of IgG B1 and IgG B11 to B lymphoma cells.
Raji cells (left panels, IgG B1) or Ramos cells (right panels, IgG B11) were incubated with increasing amounts of radioiodinated IgG B1 orradioiodinated IgG B11 protein in the presence or absence of 0.2 mg/ml of the corresponding unlabeled IgG protein. Specific binding was determined by subtracting binding in the presence of unlabeled competing protein from total binding. The amount of bound IgG B1 or IgG B11 protein increased with increasing amounts of free IgG protein with saturable binding being reached at ~30 nM IgG B1 and ~1 nM IgG B 11, respectively (upper panels). Rosenthal-Scatchard plot analysis (lower panels) demonstrated a dissociation constant of ~3 nM with 400,000 functional binding sites per Raji cell for IgG B1, and a dissociation constant of ~0.3 nM with 47,400 functional binding sites for IgG B11 (Raji cells).
Figure 6 - Binding of B1, B11, C11 lgG1 to tumour cell lines of different origin. The antigen distribution of antigens targeted by the B1, B11, and C11 antibodies on different carcinoma cell lines was investigated by flow- cytometry. Histograms show binding of Rituximab anti-CD20 Mab (first row front most peaks), B1 lgG1 (second row peaks), B11 lgG1 (third row peaks), or C11 lgG1 (fourth row back most peaks) to MCF-7 breast carcinoma, HPAC pancreatic carcinoma, PC-3 prostate carcinoma, LS174 T colorectal carcinoma, and THP-1 monocytic leukaemia cells, as indicated.
Figure 7 - B11 lgG1 apoptosis induction in carcinoma cells
The prostate carcinoma cell line PC-3 was grown in Complete Growth Medium (RPM11640, supplemented with 10 % FCS, 10 mM HEPES, and 2 mM L-Glutamine) to 80 % confluency in a 6 well plate. The prostate carcinoma cell line DU145 was grown in MEM with Earl’s salts, supplemented with 10 % FCS, 1 mM sodium pyruvate, and 1 mM non-essential amino acids and the derivate of a melanoma cell line MDA MB 435 was grown in DMEM supplemented with 10 % FCS.
For apoptosis assays cells were washed in PBS and serially diluted B11 lgG1 (or B1 IgG^ Trastuzumab or negative antibody control for controls) was added to individual wells and binding was allowed during a 1-2 h incubation at 4 °C. The cells were washed and Complete Growth Medium was added, containing crosslinking antibody, Fab’2 Goat anti-Human Fab’2, at 10 μg/ml. Cells were incubated in a humidified atmosphere, with 5 % C02 at 37 °C, for 16-24 hours. Cells were collected by trypsination and stained with Alexa Fluor 488-Annexin V (AF488-AV) and propidium iodide (PI), according to manufacturer’s instructions. The percentage apoptotic cells was determined by the formula: % apoptotic cells = 100 - % AF488 - AV/PI -/-. A) Contour plots show the relative distribution of PC-3 cells as a function of Annexin V and Propidium Iodide positivity following incubation as above with 2 μg/ml IgG B11 or IgG B1. B) Bar graph shows the mean percentage of apoptotic PC-3 cells following incubation with serially diluted B11 lgG1 or20μg/ml B1 IgG^ C) Bar graph shows the mean percentage of apoptotic MDA MB 435 cells following incubation with no antibody control, 10 μg/ml negative antibody control, serially diluted B11 IgG^ or 10 μg/ml Trastuzumb lgG1. D) Bargraph shows the mean percentage of apoptotic DU145 cells following incubation with no antibody control, 10 μg/ml negative antibody control, serially diluted B11 IgG^ or 10 μg/ml Trastuzumb lgG1
Figure 8. B1 lgG1 and B1 lgG4 induce direct cell cytotoxicity on Raji B lymphoma cells in the absence of cross-linking reagents.
Raji cells were incubated with B1 IgG^ B1 lgG4, Rituximab IgG^ or control CT-17 lgG1 at 20,. 6.7 or 2.2 μg/ml for 24 hours. Cells were harvested and viability was determined as the percentage of Annexin V and Propidium Iodide double negative cells.
Figure 9 - VH and VL sequences (nucleotide and amino acid) sequences for B1 antibody
Figure 10 - VH and VL sequences (nucleotide and amino acid) sequences for B11 antibody
Figure 11 - VH and VL sequences (nucleotide and amino acid) sequences for C11 antibody
Example 1 - Selection and Screening (Blopannlng) for apoptosis inducing antibodies, with specificity for B lymphoma associated cell surface receptors
Cell culture [0065] The cell lines used in this study were obtained from ATCC-(Manassas, VA, USA) or Deutsche Sammlung von Mikroorganismen und Zellkulturen (DSMZ) GmbH (Braunschweig, Germany) and were cultured in RPMI 1640 medium supplemented with 10 % FCS, 2 mM L-Glutamine, 10 mM HEPES and 1 mM Na pyruvate (all from Invitrogen, Carlsbad, CA, USA) unless otherwise stated. The Jurkat T leukaemia cell line (clone E6-1, TIB-152, ATCC), the B lymphoma cell lines DOHH-2 (ACC47, DSMZ), SC-1 (ACC558, DSMZ), WSU-NHL (ACC58, DSMZ), JVM-2 (ACC12, DSMZ), Jeko-1 (ACC553, DSMZ grown in 20 % FCS), Rec-1 (ACC 584, DSMZ), Sup-53 (Daibata et al. Cancer 1989;64:1248-53), RL (CRL-2261, ATCC), Granta 519 (DSMZ), NCEB-1 (Saltman et. al. Blood 1988;72:2026-30), BJAB (Menezes et al. Biomedicine 1975;22:276-84), Ramos (RL-1596, ATCC), Raji (CCL-86, ATCC), Daudi (CCL-213, ATCC), CL-01 (Cerutti et al. J Immunol 1998;160:2145-57), the pre B cell lymphoma KM-3/Reh (CRL-Ő286, ATCC) and the multiple myeloma MC/CAR (CRL-8083, ATCC, grown in IMDM (Invitrogen) supplemented with 20 % FCS) were all free of mycoplasma and cultured in a humidified atmosphere at 37 °C, using a 5 % C02 atmosphere. The cells were maintained at 2 X 105-1 X 106 cells/ml.
Jurkat cell membrane vesicle preparation [0066] Jurkat cells were harvested by centrifugation at 300 X g for 15 min in 500 ml buckets (Corning Inc. Life Sciences, New York, USA), washed in Dulbecco’s PBS (Invitrogen), and resuspended in buffer A (1 mM NaHCOs, 1.5 mM MgAc, pH 7.4). Cell concentration was approximately 5 X 107 Jurkat cells/ml (5 X 109 cells in 100 ml Buffer A).
[0067] Cell disruption was achieved by hypo-osmotic shock treatment (Buffer A) on ice for 10-30 min and subsequent nitrogen cavitation in a Nitrogen cavitation bomb (Parr Instrument Company, Moline, IL, USA). Cells were kept at a constant pressure of 40 bar (4,000 kPa) for 15 min at 0 °C.
[0068] Disrupted cells were collected in a 250 ml Sarstedt tube (Sarstedt AG & Co, Nümbrecht, Germany) containing 500 μΙ 0.5 M EDTA to yield a final EDTA concentration of 2.5 mM. Addition of EDTA prevents aggregation of membrane vesicles. The homogenate (100 ml) was divided between 4 X 25 ml Beckman thick-walled rotor tubes (Beckman Coulter, Inc., Fullerton, CA, USA), which were centrifuged for 10 min at 1900 X g (4,000 rpm in an Sorvall SS34 rotor) at 4 °C to remove unbroken cells, nuclei, and heavy mitochondria.
[0069] The supernatant was collected and pelleted material was resuspended in 25 ml of 1 mM NaHC03 buffer containing 1 mM EDTA and was re-centrifuged (further recovery of pelleted crude Jurkat membranes). Jurkat membranes were pooled with membranes from the first centrifugation. Supernatants containing crude Jurkat membrane vesicles were ultra centrifuged using a Beckman Type45Tirotorat40,000 rpm (approx. 200,000 x g)for2.5 hat4°C. Supernatants were poured off and remaining buffer was removed by tipping the tube edge against a tissue (e.g. Kleenex™).
[0070] The crude membrane pellet was transferred to a Dounce homogeniser with the aid of a metal bar and was resuspended in 2.5 ml HES buffer (10 mM Hepes, 1 mM EDTA, 0.25 M sucrose, pH 7.4) by several careful strokes in the homogenizer. A membrane suspension concentration equivalent of 2 X 109 cells/ml containing 80- 100 mg protein was, thus, achieved.
Selection of phage Abs by whole celllcell membrane vesicle competition biopanning [0071] Approximately 2 X 1013 phage particles were pre-warmed at 37 °C for 15 min with intermittent mixing, centrifuged for 15 min at 14,000 X g to remove precipitates, and the supernatant was transferred to afresh Eppendorf tube. Nonfat dry milk was added to a final concentration of 2 % (w/v). Jurkat membrane vesicle preparations derived from 2 x 109 cells (round 1 selection; 2 x 108 cells round 2 and 3 selections) were thawed on ice, and were mixed with the blocked phage particles. The mixture was incubated for 15 min on ice.
[0072] 5 X 107 (5 X 106 2nd and 3rd rounds) Ramos cells were harvested by centrifugation at 1,200 rpm for 6 min at 4 °C. Supernatant was discarded and Ramos cells were resuspended in the milk-phage-Jurkat membrane vesicle mixture. The suspension was incubated at 10 °C under slow end-over-end rotation for 4 h.
[0073] The cell/ cell membrane vesicle/ phage mixture was transferred to a 15 ml Falcon tube (BD Biosciences, Bedford, MA, USA), containing 0.5 ml 100 % (trypan blue stained) Ficoll-Paque PLUS (Amersham Biosciences, Uppsala, Sweden) at the bottom, and 9.5 ml overlaid 40 % (v/v) Ficoll in 2 % (w/v) BSA/PBS (Ficoll-pillar). The tube was centrifuged at 1,500 rpm for 10 min at 4 °C. The tube was removed from the centrifuge and the tube cap was screwed on and sealed airtight.
[0074] The bottom "tip" of the Falcon tube containing 100 % Ficoll was chopped off using a cigar-chopper. Thus, very high-density material including membrane vesicle sheets and cell nuclei were eliminated from the tube. The tube cap was then carefully opened disrupting the vacuum inside the tube and allowing liquid to be expelled drop-wise through the opening at the (cut off) tube bottom.
[0075] The harvested cell suspension was washed once in PBS to remove excess Ficoll. The pellet was resuspended in 1 ml PBS (not performed following final wash) and the suspension was reloaded on top a fresh Ficoll-pillar and the washing procedure was repeated (twice in rounds 2 and 3).
[0076] Phage were eluted from cells by addition of 150 μΙ of 76 mM citric acid (pH 2.5) in PBS followed by incubation at room temperature for 5 min. The mixture was neutralized by addition of 200 μΙ of 1 M Tris-HCI, pH 7.4. Supernatants containing eluted phage were saved following pelleting of cells at 300 X g for 5 min. Further elution of phage was by resuspension and incubation of the cell pellet in 1 ml trypsin at RT for 10 min.
[0077] Following inactivation with 40 μ| 1 mg/ml aprotinin, cells were centrifuged and supernatant containing eluted phage was saved. Eluted phage were used to infect Escherichia coli HB101F’ and the bacteria were plated on TB medium containing appropriate antibiotics and glucose. Bacterial colonies were counted, scraped from the plates, and used as inoculums for the next round of panning.
Conversion to scFv format, scFv expression, purification, and analysis of cell binding [0078] The phagemid pool obtained following three rounds of selection was digested with Eag\ to remove the gene III. The resulting vector was re-ligated. Vectors containing re-ligated uncut gene III fragments were linearized by digestion with EcoRI enzyme. The scFv vector pool thus generated was used to transform E. coli TOP10 cells essentially as described earlier (Soderlind et al. Nat Biotechnol 2000;18:852-6.).
[0079] Bacteria were plated on large 500 cm2 agar plates and individual clones were picked, transferred to 96-well plates, and expressed in TB medium by over night culture at 37 °C, 220 rpm using an automated system (Hallborn Biotechniques 2002;Suppl:30-7.). Recombinant scFv fragments were produced in TB medium containing appropriate antibiotics.
[0080] For primary screening of scFv clone binding to target Ramos cells and Jurkat non-target cells, 5,000 Ramos or Jurkat cells were incubated with either of 960 scFv clones, derived from the 3rd round of selection and produced as described above. Cells were incubated with 0.5 μg/ml anti-6xHis mAb (R&D Systems, Minneapolis, MN, USA) and 0.7 μg/ml Cy5-conjugated Goat anti-mouse reagent (Amersham Biosciences). Cell binding was analysed in an 5200 Cellular Detection System Fluorescence Macroconfocal High Throughput Screening (FMAT) instrument (Applied Biosystems, Foster City, CA, USA).
[0081] Following primary screening, seventy two bacterial clones were picked randomly (i.e. irrespective of target cell vs. non-target cell reactivity in the primary screening) for DNA sequencing as described previously (Soderlind et al. Nat Biotechnol 2000;18:852-6.) (Soderlind et ai., 2000). Forevaluation of cell surface binding by flow-cytometry, Ramos and Jurkat cells (both added at 2 x 105 cells per test) were incubated with individual scFv clones at a concentration of 2-10 μg/ml in PBS (Invitrogen) containing 0.5 % w/v BSA (DPBS-B) for 1 h.
[0082] Cells were washed by centrifugation at 300 X g for 6 min. Cells were then incubated with FITC-conjugated CD 19 mAb and PE-conjugated CD3 mAb(BD) enabling subsequent identification of target and non-target cells, respectively. Detection of scFv binding was achieved by incubation with RPE-Cy5-streptavidin (Dako Cytomation, Glostrup, Denmark) following incubation with biotinylated anti-6xHis mAb. Cells were incubated with secondary and tertiary reagents for 40 min, and 15 min respectively. All incubations were performed on ice using ice-cold solutions.
Differential whole cellI cell membrane vesicle panning [0083] The present study utilized a novel panning protocol to isolate antibodies that target differentially expressed antigens in their native cell surface configuration. Following three rounds of competition biopanning, using whole Ramos B lymphoma cells and membrane vesicles derived from Jurkat T leukaemia cells, recombinant phage scFv were isolated. These were converted to soluble scFv and expressed in E. coli TOP10 cells.
[0084] Recombinant scFv were incubated with target (Ramos) or non-target (Jurkat) whole cells and examined for cell binding. The specificity for target cell antigens of the antibody clones was striking, since 482 scFv clones expressed were shown to bind selectively to Ramos target cells at intensities ranging from weak to very strong (Fig 1 A). Only two clones were identified that weakly stained non-target Jurkat cells (Fig 1A).
[0085] We next determined the genotype diversity of isolated phage displayed scFv. Seventy-two scFv clones were randomly picked (i.e. irrespective of binding tropism as determined in the primary screening) for DNA sequencing.
[0086] The clones were simultaneously re-expressed and re-evaluated for target cell specificity (Ramos vs. Jurkat) by FMAT technology, as described (Fig 1 B). Seven different antibody genotypes were identified, as determined by their different CDRH3 and CDRL3 sequences (data not shown).
[0087] The high specificity of anti-Ramos scFv was confirmed by three colour flow-cytometric analysis, following incubation with equal numbers of Ramos and Jurkat cells and detection of scFv binding by means of anti-tag antibody (Fig. 1C).
[0088] Target and non-target cells were defined by CD19 and CD3 expression, respectively, using fluorochrome conjugated CD specific monoclonal antibodies. The seven genotypically unique scFv clones showed high and variable binding intensities to target Ramos cells, but no binding to the non-target Jurkat cells, as compared to the negative control scFv.
Apoptosis assay [0089] Lipopolysaccharide levels of recombinantly produced scFv fragments were reduced using Detoxigel columns according to manufacturer’s instructions (Pierce Biotechnology, Rockford, IL, USA). Remaining endotoxin levels were quantified by the LAL-amebocyte lysate assay (Cambrex Bioscience, Walkersville, MD, USA).
[0090] All scFv samples were found to contain less than 0.1 lU/ml of lipopolysaccharide. The chimeric anti-CD20 antibody Mabthera™ (Rituximab) was purchased from Lund University Hospital (Lund, Sweden). 2 X 105 B lymphoma cells (Raji or Ramos) or Jurkat T cells were incubated with serially diluted and detoxified scFv’s in culture medium for 1 h on ice.
[0091] Cells were sequentially incubated with secondary anti-6xHis mAb (5 ^g/ml), and tertiary Goat Fab’2 anti-mouse Fab’2 antibody (Jackson ImmunoResearch Laboratories, Inc., West Grove, PA, USA). Intermittent washings ensured removal of excess unbound antibody reagent. Cells were incubated at 37 °C in a humidified atmosphere of 5 % C02for 24 h.
[0092] When whole IgGs were used for apoptosis induction, cross-linking reagent was replaced by goat Fab’2 antihuman Fey antibody (Jackson ImmunoResearch) with minimal cross-reactivity with non-IgG antibody isotypes (to avoid unspecific cross-linking of endogenous B lymphoma associated surface immunoglobulins) and incubated, as described above, for 6 h.
[0093] Apoptotic cells were, unless otherwise stated, detected by combined staining with Annexin V Alexa Fluor 488 (AV) and Propidium Iodide (PI) (both from Molecular Probes, Invitrogen) and subsequent flow-cytometric analysis, Cells were defined as viable (AV-/PI-), early apoptotic (AV+/ PI-) or late apoptotic/necrotic (AV+/PI+). AV and PI signals were recorded in the FL1 and FL2 or FL3 channels (as indicated in the text), respectively, using a FACSCalibur instrument (BD Biosciences).
[0094] In order to investigate the functionality of the isolated scFv we set up a high throughput apoptosis screening assay, based on sequential incubation and washing of cells with scFv and cross-linking reagent. The dependence on scFv clone and concentration in the apoptosis assay is demonstrated in Fig. 2A-C, where the apoptotic effect of selected scFv clone B1 is compared to the - effect of scFv clone F1 which shows no induction of apoptosis. Jurkat cells lacking target antigen expression did not die from apoptosis after treatment with any of the examined scFv demonstrating that apoptosis induction depended on binding to target antigen (data not shown).
[0095] Using the established scFv-apoptosis assay, we screened clones for apoptosis on Ramos and Raji B lymphoma cells. scFv-induced apoptotic effects were compared to that induced by Rituximab anti-CD20 mAb (Fig. 2D). Three scFv clones - B1, B11 and C11 - were identified that induced significant apoptosis on both Ramos and Raji cells (Fig. 2D and E). Induction of apoptosis by scFv on Raji cells correlated with binding to these cells (Fig. 2D), since scFv clones that failed to bind Raji cells did not induce apoptosis.
[0096] The B1, B11 and C11 clones were transferred to fully human lgG1 antibodies. Both their specificity and functionality remained intact after reformatting, as demonstrated by their strong binding and potent cytotoxicity towards a broad panel of B lymphoma cell lines (Table 1). Notably, apoptosis induction was rapid with maximal percentage of annexin V positive apoptotic cells being reached already after three to six hours in several cell lines (Table 1 and data not shown).
IgG production and endotoxin screening assays [0097] scFv antibody fragments were converted to full-length human IgG 1 λ format via cloning into a modified pCDNA3 vector (Norderhaug et al. J Immunol Methods 1997;204:77-87.), and transiently transfected into HEK293 cells using Lipofectamine 2000 reagent according to manufacturer’s instructions (Invitrogen).
[0098] Fluman IgG was purified from spent cultivation medium on a MabSelect protein A column (Amersham Biosciences). The purity of preparations was >98% as determined by SDS-PAGE analysis. Antibody preparations were screened and found to contain < 0.1 lU/ml endotoxin at concentrations used in the present study, and as determined by the LAL amoebocyte lysate test (Cambrex Bioscience).
Example 2 -Analysis of antibody specificity
Antigen Identification [0099] The identity of the targeted antigens was determined by immunoprécipitation of B lymphoma cell lysates. Cells (50-600 X 106 per ml lysis buffer, depending on antibody and cell line) were harvested by centrifugation, washed twice in PBS and incubated for 15 min in Lysis Buffer (25 mM Tris-HCI, pH 7.5, 150 mM NaCI, 5 mM EDTA, and Complete EDTA-free Protease inhibitor cocktail (Roche Diagnostics GmbH, Mannheim, Germany)) containing the detergent Triton X-100 (Sigma-Aldrich, St. Louis, MO, USA) at 0.5 % v/v.
[0100] Cellular debris was spun down at 16,000 X g for 15 min in a conventional table-top centrifuge and the soluble proteins were pre-cleared with Protein A Sepharose 4 Fast Flow (Amersham Biosciences) (1/10 volume of reaction) for 1 h on rotation. For every sample, 1 ml of pre-cleared cell lysate was immunoprecipitated for 2 h by 20-100 μg of any of the human antibodies. Protein A Sepharose 4 Fast Flow was added again and incubated for 30 min, where after the immuno-complexes were washed extensively in lysis buffer, boiled for 5 min, and finally resuspended in Sample Buffer (1X NuPAGE LDS Sample Buffer, 1X NuPAGE Sample Reducing Agent) and separated in a NuPAGE Novex 4-12 % Bis-Tris Gel (all from Invitrogen).
[0101] After staining (Simply Blue Safestain, Invitrogen), protein bands of interest were excised from the SDS-PAGE and subjected to tryptic digestion, as described (Edvardsson et al. Electrophoresis 1999;20:935-42.).
[0102] Briefly, gel plugs were destained and equilibrated by washing three times with 200 μΙ 50 % acetonitril (ACN) under agitation. After drying in a SpeedVac concentrator (Savant, Farmingdale, NY, USA) for 15 min, samples were reduced by addition of 25 μ110 mM DTT /100 mM NH4HC03 and incubated for 56 °C for 1 h and alkylated by addition of 25 μΙ 55 mM iodoacetamide /100 mM NH4HC03 followed by incubation for 45 min at room temperature.
[0103] After two additional 10 min washing steps in 100 mM NH4HC03 followed by one wash in 50 % v/v ACN, the gel pieces were dried in a SpeedVac concentrator and re-swelled and digested in 15 μΙ of 15 ng/μΙ trypsin (Promega Corporation, Madison, Wl, USA) in 25 mM NH4HC03 at 37 °C over night. Peptides were extracted by addition of 50 % v/v ACN / 1 % v/v TFA and 10 min incubation at RT. 1 μΙ of the extract was spotted onto MALDI sample plates and allowed to dry. 1 μΙ matrix solution (5 mg/ml alpha-cyano-4-hydroxy cinnamic acid (CFICA) in 75 % v/v ACN /1 % v/v TFA) was spotted on top of the peptides.
[0104] Peptide masses were determined using an Applied Biosystems 4700 Maldi Workstation. The proteins were identified by peptide mass fingerprint database searching using Mascot search tools (Matrixscience, UK). Antigen specificities of clones B10, C10, and G12 were identified using similar methodology, except scFv’s and anti-His coated magnetic microbeads (Miltenyi Biotec GmbFI, Bergisch Gladbach, Germany) were used for immunoprécipitations.
[0105] Following conversion to the full antibody format B1, B11 and C11 IgG were used to precipitate antigens from Raji and Ramos B lymphoma cells. IgG B1 precipitated two bands of approximately 28 and 34-kDa, respectively (Fig. 3A, lane 1). Gel slices containing these bands were prepared and digested with trypsin and analysed by mass spectrometry identifying HLADR/DP as the target antigen.
[0106] The specificity of IgG B1 for FILA-DR/DP was verified both by western blotting and detection of HLA-DR/DP protein, using a commercially available monoclonal antibody, and by blocking of B1 IgG binding following pre-incubation of cells with a commercially available HLA-DR specific monoclonal antibody (Fig. 3B).
[0107] The identities of the IgG B11 and C11 defined antigens were established using similar methodology. IgG C11 was found to precipitate a 68 kDa protein band identified as the membrane bound form of the B cell receptor μ chain (Fig. 3A, lane 3). IgG B11 precipitated a 90 kDa protein band that was identified as the intercellular cell adhesion molecule-1 (ICAM-1) (Fig. 3A, lane 2). The specificities of IgG B11 for ICAM-1, and of C11 IgG for IgM, were confirmed by MS-MS analysis, antibody blocking studies (Fig. 3B), and western blot analysis (data not shown) using commercially available antibodies.
[0108] Specificities of clones B10, C10, and G12 were determined, using scFv and anti-His coated magnetic microbeads for immunoprécipitation. The three scFv clones precipitated a protein band of 68 kDa, and MS-analysis of trypsin digested gel slices containing these bands revealed their specificity for surface IgM. Presumably, these antibodies recognize the Ramos IgM idiotype, since neither of them cross-react with peripheral blood B lymphocytes or other IgM positive B cell lines.
Example 3 -Analysis of antibody affinities
In vitro iodination of B1 and B11 Immunoglobulins [0109] Iodination of 1 mg/ml of lgG1 B1 or lgG1 B11 proteins with [125l] Nal was performed in PBS for 10 min using lodogen pre-coated iodination tubes (Pierce). Free [125l] Nal was removed by desalting on PD-10 columns (Amersham Biosciences), yielding specific radioactivities in the range of 1000-1600 cpm per ng protein. [125l] lgG1 B1 and [125l] lgG1 B11 was used for determination of antibody affinities.
Determination of IgG B1 and IgG B11 affinity constants [0110] Radioiodinated IgG B1 or IgG B11 was incubated with B lymphoma cells in DPBS-B-hlgG (DPBS-B containing 0.2 mg/ml human IgG) for 2 h on ice with intermittent mixing. Non-specific binding was determined in the presence of 0.2 mg/ml unlabeled IgG B1 or IgG B11 protein, as appropriate. Analysis was performed in triplicates.
[0111] Cells were loaded on top 40 % v/v Ficoll/DPBS-B cushions in individual tubes and were centrifuged at 400 X g for 6 min at 4 °C. Samples were frozen at -80 °C. Cell pellets and cell supernatants were isolated and analysed separately for 125l-lgG protein content in a gamma counter, following cutting of the tubes in half.
[0112] Antibody affinity constants (Kd values) and epitope numbers per cell were determined from Scatchard plot analysis according to Rosenthal et al. (Anal Biochem 1967;20:525-32), Bylund and Yamamura (Methods in Neurotransmitter Analysed. New York: Raven Press Ltd., 1990), and Marquardt (J. Soc. Indust. Appl. Math 1963;11:431-41), as previously described (Brix et al. J. Clin. Invest. 1998;102:283-93).
[0113] IgG B1 and IgG B11 binding to HLA-DR and ICAM-1 was characterised by incubating the radio-iodinated proteins with Raji or Ramos cells in the presence or absence of 0.2 mg/ml of the corresponding unlabeled IgG protein at 4 °C. The specific binding of [125l]lgG to the cell surface was calculated by subtracting non-specific binding (binding in the presence of excess unlabeled IgG) from the total binding.
[0114] Saturation of specific IgG B1 binding to Raji cells was reached at ~30 nM IgG B1 (Fig. 5). Rosenthal-Scatchard plot analysis revealed a dissociation constant of ~3 nM with 400,000 functional binding sites per Raji cell, assuming a bivalent epitope-IgG interaction (Fig. 5). Similarly, the dissociation constant of IgG B11 was determined to -0.2 nM with 47,400 receptors per Ramos cell.
Example 4 - ICAM-1 is a B lymphoma associated antigen with apoptosis inducing properties
Flow-cytometric analysis of IgG binding to Ramos cells [0115] Ramos cells (13 x 106) were stained with CD45-PerCp-Cy5.5 mAb by incubation on ice for 45 min, washed in DPBS-B, and kept on ice until mixing with unlabeled purified PBLs.
[0116] Buffy coats from two healthy volunteers were obtained from the Lund University Hospital. Buffy coats were diluted 1:2 in PBS and washed by centrifugation at 500 X g (1500 rpm Beckman Spinchron centrifuge) for 10 min, complete aspiration of the supernatant and resuspension in DPBS containing 1 % heat inactivated FCS (DPBS-HI). Washing was repeated twice. Red blood cells were lysed by incubation with red blood cell lysing solution (BD Biosciences) for 15 min at RT. Cells were washed by centrifugation at 60 X g (667 rpm Beckman spinchron centrifuge) for 10 min and the supernatant was carefully aspirated. Cells were counted in a Bürker chamber following staining with trypan blue reagent (Invitrogen) and exclusion of dead cells, washed in DPBS-HI, pelleted, and resuspended in DPBS-B containing 200 μg/ml human purified IgG (blocking of Fc receptors).
[0117] For each donor and test condition, approximately 2.5 X 106 leukocytes were mixed with 1.6 X 105 PerCpCy5.5 pre-labelled Ramos cells. Mouse monoclonal CD3-FITC, CD56-PE, and CD19-PerCpCy5.5 antibodies (BD Biosciences) were added and the mixtures were incubated on ice until addition of labelled human IgG. Labelling of n-CoDeR human IgG antibodies and positive control anti-CD20 mouse-human chimeric antibody Rituximab with AF647 Fab fragments (Molecular Probes, Invitrogen) was performed according to manufacturer’s instructions.
[0118] Briefly, 4 μg of each of IgG B1, B11, C11, and Rituximab antibodies were incubated with 20 μΙ of AF647-Fab labelling reagent for 5 min at RT. Following addition of 20 μΙ human IgG blocking reagent and a further incubation for 5 min, AF647-labeled IgG was three-fold serially diluted in DBPS-B, and diluted IgG proteins were added to the mixed Ramos/PBL cell solutions.
[0119] Samples were incubated for 1 h, washed, resuspended in DPBS-B, and analysed for binding to different cell subpopulations by flow-cytometry, following appropriate calibration and compensation of the instrument for four-colour analysis. Ramos cells were identified as the PerCpCy5.5h'9h population distinct from the B lymphocyte PerCpCy5.5low population.
Immunohistochemistry [0120] Cryopreserved lymph node biopsies of patients with Anaplastic Large Cell B lymphoma (one patient), Centro-blastic/Centrocytic B non-Hodgkin lymphoma (three patients), and B cell chronic lymphocytic leukaemia (one patient) were obtained from the Department of Pathology at Lund University (Lund, Sweden). Eight-micrometer sections of cryopreserved tissue were fixed in acetone for 10 min at 4 °C. Endogenous biotin-binding activity was blocked by sequential treatment with Avidin and Biotin (Avidin/Biotin blocking kit, Invitrogen) for 20 min each.
[0121] Tissues were incubated with 5 μg/ml control scFv or B11 scFv for 1 h. Following washing, sections were incubated with biotin-conjugated mouse anti-His mAb (R&amp;D Systems) for 30 min. scFv binding was detected following treatment with ABC Complex/ HRP reagent (DakoCytomation) for 30 min, and subsequent incubation with DAB for 5 min.
[0122] Sections were photographed using a Leica DC 300F digital camera mounted on top of a Leica DMR light/flu- orescence microscope.
[0123] Handling of human tissue followed the recommendation of the local Ethics Committee at Lund University Hospital.
Mitochondrial membrane depolarisation assay [0124] Mitochondrial membrane depolarisation was analysed as previously described (Kim et al. Mol Biol Cell 2004;15:420-34). Briefly, antibody-treated cells were mixed with JC-1 reagent (Molecular Probes) at 5 μg/ml and incubated for 30 min at RT. Cells were washed twice in ice-cold PBS and resuspended in 300 μΙ PBS and analysed on a FACS Aria (BD Biosciences). The green and red fluorescence was collected through 494/518 nm (FL-1) and 595/615 nm (FL-2) bandpass filters, respectively.
[0125] ICAM-1 is a glycoprotein of the immunoglobulin superfamily (Marlin et al. Cell 1987;51:813-9) capable of inducing bi-directional signalling (Roth lein et al. J Immunol 1994;152:2488-95; Vyth-Dreese étal. Blood 1995;85:2802-12). ICAM-1 has not previously been demonstrated to be involved in programmed death in B lymphoma cells.
[0126] Therefore, we wanted to confirm that IgG B11 induced cell death was an active process, by means other than cell membrane phosphatidyl serine translocation.
[0127] Mitochondrial membrane depolarisation was chosen as a validation of apoptosis, since this is a common feature of caspase dependent and caspase independent apoptosis that may be monitored by cell staining with 5,5’,6,6’-tetra-chloro-1,1’,3,3’-tetraethylbenzimidazolyl-carbocyanine iodide (JC-1 reagent).
[0128] In accordance with our Annexin V/propidium iodide assay (Fig. 4A, upper panel), IgG B11 was found to induce mitochondrial membrane depolarisation in CL-01 B lymphoma cells, as determined by flow-cytometric analysis following staining with JC-1 reagent (Fig. 4A, lower panel).
[0129] In order to exclude the possibility that ICAM-1 expression was an in vitro artefact, resulting from a general up-regulation during cell culture, we examined the binding of IgG B11 to tissue obtained from five different patients with different B lymphoma tumours.
[0130] By immunohistochemistry, IgG B11 showed strong binding to the five lymphoma tissues (Fig. 4B), at intensities comparable to, or slightly lower than, the anti-FILA-DR/DP antibody IgG B1 (Table 2).
[0131] We next examined the binding of IgG B11 to B lymphoma versus resting peripheral blood leukocytes. Ramos was chosen as a representative B lymphoma cell line, based on its low-end epitope expression yet significant sensitivity to B11 induced apoptosis. Flow-cytometric analysis, following mixed incubation of pre-labelled Ramos cells with whole blood peripheral blood leukocytes and either of IgG B1, B11 orC11 antibodies, revealed that IgG B11 showed strong binding to Ramos cells.
[0132] Even more importantly, B11 demonstrated the greatest differential binding (strongest antigen up-regulation) of the three antibodies to Ramos B lymphoma cells versus normal peripheral blood leukocytes (Fig. 4C. and data not shown). IgG B11 binding peaked already at 0.1 μg/ml and was 3.7-fold up regulated on Ramos versus monocyte cells (MFI 654 versus 176), 8.3-fold up regulated on Ramos versus peripheral blood B lymphocytes (MFI 654 versus 78), and 23-fold up regulated compared to NK cells. Binding to other monitored peripheral blood leukocyte subsets was negative.
Table 2. ICAM-1 is strongly expressed in B lymphoma tissue of different origin
Example 5 - Antigen distribution ofB1, B11, C11 lgG1 on tumour cell lines of various origins, as determined by flow cytometry.
[0133] The antigen distribution of human antibody targeted antigens, mainly for B 11, on different carcinoma cell lines was investigated. Cells (MCF-7 and MDA MB 435S breast carcinoma, JAR and JEG-3 chorio-carcinoma, A549 lung carcinoma, TCC-SUP urinary bladder carcinoma, MDA MB 435 melanoma, FIPAC, PANC-1 and BxPC-3 pancreatic carcinoma, PC-3 and DU 145 prostate carcinoma, LS174 T, CaCo2, and Lovo colorectal carcinoma, and THP-1 monocytic leukaemia cells), were washed in PBS, and resuspended at 4 x 106 cells/ml in Complete Medium (200,000 cells/50 μΙ sample). B1 IgG^ B11 IgG^ C11 IgG^ negative control FITC-8 IgG^ and Rituximab anti-CD20 mAb was 3-10-fold serially diluted (10-0.1 pg/ml) in Complete Medium (50 μΙ/sample). Cells were incubated with either of the antibodies for 1 hour on ice, washed by resuspension in PBS/BSA 0.5 %, centrifuged at 1200 rpm for 5min, and complete aspiration of the supernatants was undertaken. Cells were incubated with PE-conjugated Goat F(ab’)2 anti-Fluman IgG (Caltag Laboratories, Cat no: F110104), diluted 1/50 in PBS/BSA 0.5 %, for 30 min, on ice. Following resuspension of in 300 μΙ PBS/BSA 0.5 %, cells were analysed for IgG binding using a FACScan instrument.
[0134] PC-3 prostate carcinoma cells showed strong expression of ICAM-1 as demonstrated by the strong binding of B11 IgG to these cells (Fig. 6). MCF-7 breast carcinoma, FIPAC pancreatic carcinoma, and LS174T colorectal carcinoma cells were also found to express ICAM-1 albeit at lower intensity compared to the prostate cancer cells. In contrast, TFHP-1 monocytic leukaemia cells did not express ICAM-1. All carcinoma cell lines initially tested were found negative for CD20, FI LA-DR/DP, and IgM expression as demonstrated by the lack of binding of Rituximab IgG, B1 IgG, and C11 IgG, respectively. Further studies on additional carcinoma cells lines indicated that all carcinoma cells examined were positive for ICAM-1 expression (Table 3).
Example 6 - B11 lgG1 apoptosis induction in carcinoma cells [0135] B11 lgG1 was shown in example 5 to bind strongly to carcinoma cells. The present example examined the apoptosis inducing properties of this antibody on carcinoma cells.
[0136] Cells were seeded in 6 well plates with Complete Growth Medium three days before the onset of the experiment. Cells were between 50-75 % confluent at the time of the experiment. Cells were washed with ice-cold PBS and incubated with serially diluted (20- 0.02 μg/ml as indicated in the figures, in 1 ml Complete Growth Medium) B11 IgG^ 20 μg/ml control B1 IgG^ 10μg/ml negative control IgGi or 10 μg/ml Trastuzumab lgG1 as indicated at 4 °C for 1-2 hours. Cells were washed with ice-cold PBS and secondary F(ab’2) Goat anti-Human F(ab’2) antibody (diluted in Complete Growth Medium to 10 μg/ml) was added. Cells were incubated at 37 °C, in a humidified atmosphere of 5 % C02 for 16-24 hours. Total cells were collected by first isolating the supernatant, followed by PBS wash and trypsination of remaining adherent cells. The enzymatic reaction was terminated by resuspension in PBS containing 10 % heat-inactivated fetal calf serum. Cells were washed in ice-cold PBS, subjected to Annexin V / propidium iodide staining, and analysed for viability/ apoptosis as described in example 5 above.
[0137] The B11 lgG1 was shown to induce apoptosis in the carcinoma cell lines in a specific and titratable manner (Figure 7). Control IgG B1, which did not bind to PC-3 cells (see example 5), also did not induce apoptosis in PC-3 cells. Negative control lgG1 or Trastuzumab lgG1 were not able to induce apoptosis in DU145 or MDA MB435 cells.
Example 7- Pharmaceutical formulations and administration.
[0138] A further aspect of the invention provides a pharmaceutical formulation comprising a compound according to the first aspect of the invention in admixture with a pharmaceutically or veterinarily acceptable adjuvant, diluent or carrier.
[0139] Preferably, the formulation is a unit dosage containing a daily dose or unit, daily sub-dose or an appropriate fraction thereof, of the active ingredient [0140] The compounds of the invention will normally be administered orally or by any parenteral route, in the form of a pharmaceutical formulation comprising the active ingredient, optionally in the form of a non-toxic organic, or inorganic, acid, or base, addition salt, in a pharmaceutically acceptable dosage form. Depending upon the disorder and patient to be treated, as well as the route of administration, the compositions may be administered at varying doses.
[0141] In human therapy, the compounds of the invention can be administered alone but will generally be administered in admixture with a suitable pharmaceutical excipient, diluent or carrier selected with regard to the intended route of administration and standard pharmaceutical practice.
[0142] For example, the compounds of the invention can be administered orally, buccally or sublingually in the form of tablets, capsules, ovules, elixirs, solutions or suspensions, which may contain flavouring or colouring agents, for immediate-, delayed- or controlled-release applications. The compounds of the invention may also be administered via intracavemosal injection.
[0143] Such tablets may contain excipients such as microcrystalline cellulose, lactose, sodium citrate, calcium carbonate, dibasic calcium phosphate and glycine, disintegrants such as starch (preferably corn, potato or tapioca starch), sodium starch glycollate, croscarmellose sodium and certain complex silicates, and granulation binders such as polyvinylpyrrolidone, hydroxypropylmethylcellulose (HPMC), hydroxy-propylcellulose (HPC), sucrose, gelatin and acacia. Additionally, lubricating agents such as magnesium stearate, stearic acid, glyceryl behenate and talc may be included.
[0144] Solid compositions of a similar type may also be employed as fillers in gelatin capsules. Preferred excipients in this regard include lactose, starch, a cellulose, milk sugar or high molecular weight polyethylene glycols. For aqueous suspensions and/or elixirs, the compounds of the invention may be combined with various sweetening or flavouring agents, colouring matter or dyes, with emulsifying and/or suspending agents and with diluents such as water, ethanol, propylene glycol and glycerin, and combinations thereof.
[0145] The compounds of the invention can also be administered parenterally, for example, intravenously, intra-arterially, intraperitoneally, intrathecally, intraventricularly, intrasternally, intracranially, intra-muscularly or subcutaneously, or they may be administered by infusion techniques. They are best used in the form of a sterile aqueous solution which may contain other substances, for example, enough salts or glucose to make the solution isotonic with blood. The aqueous solutions should be suitably buffered (preferably to a pH of from 3 to 9), if necessary. The preparation of suitable parenteral formulations under sterile conditions is readily accomplished by standard pharmaceutical techniques well-known to those skilled in the art.
[0146] Formulations suitable for parenteral administration include aqueous and non-aqueous sterile injection solutions which may contain anti-oxidants, buffers, bacteriostats and solutes which render the formulation isotonic with the blood of the intended recipient; and aqueous and non-aqueous sterile suspensions which may include suspending agents and thickening agents. The formulations may be presented in unit-dose or multi-dose containers, for example sealed ampoules and vials, and may be stored in a freeze-dried (lyophilised) condition requiring only the addition of the sterile liquid carrier, for example water for injections, immediately prior to use. Extemporaneous injection solutions and suspensions may be prepared from sterile powders, granules and tablets of the kind previously described.
[0147] For oral and parenteral administration to human patients, the daily dosage level of the compounds of the invention will usually be from 1 mg/kg to 30 mg/kg. Thus, for example, the tablets or capsules of the compound of the invention may contain a dose of active compound for administration singly or two or more at a time, as appropriate. The physician in any event will determine the actual dosage, which will be most suitable for any individual patient, and it will vary with the age, weight and response of the particular patient. The above dosages are exemplary of the average case. There can, of course, be individual instances where higher or lower dosage ranges are merited and such are within the scope of this invention.
[0148] The compounds of the invention can also be administered intranasally or by inhalation and are conveniently delivered in the form of a dry powder inhaler or an aerosol spray presentation from a pressurised container, pump, spray or nebuliser with the use of a suitable propellant, e.g. dichlorodifluoromethane, trichlorofluoromethane, dichlo-rotetrafluoro-ethane, a hydrofluoroalkane such as 1,1,1,2-tetrafluoroethane (HFA 134A3 or 1,1,1,2,3,3,3-heptafluoro-propane (HFA 227EA3), carbon dioxide or other suitable gas. In the case of a pressurised aerosol, the dosage unit may be determined by providing a valve to deliver a metered amount. The pressurised container, pump, spray or nebuliser may contain a solution or suspension of the active compound, e.g. using a mixture of ethanol and the propellant as the solvent, which may additionally contain a lubricant, e.g. sorbitan trioleate. Capsules and cartridges (made, for example, from gelatin) for use in an inhaler or insufFlator may be formulated to contain a powder mix of a compound of the invention and a suitable powder base such as lactose or starch.
[0149] Aerosol or dry powder formulations are preferably arranged so that each metered dose or "puff" delivers an appropriate dose of a compound of the invention for delivery to the patient. It will be appreciated that the overall daily dose with an aerosol will vary from patient to patient, and may be administered in a single dose or, more usually, in divided doses throughout the day.
[0150] Alternatively, the compounds of the invention can be administered in the form of a suppository or pessary, or they may be applied topically in the form of a lotion, solution, cream, ointment or dusting powder. The compounds of the invention may also be transdermally administered, for example, by the use of a skin patch. They may also be administered by the ocular route, particularly for treating diseases of the eye.
[0151] For ophthalmic use, the compounds of the invention can be formulated as micronised suspensions in isotonic, pH adjusted, sterile saline, or, preferably, as solutions in isotonic, pH adjusted, sterile saline, optionally in combination with a preservative such as a benzylalkonium chloride. Alternatively, they may be formulated in an ointment such as petrolatum.
[0152] For application topically to the skin, the compounds of the invention can be formulated as a suitable ointment containing the active compound suspended or dissolved in, for example, a mixture with one or more of the following: mineral oil, liquid petrolatum, white petrolatum, propylene glycol, polyoxyethylene polyoxypropylene compound, emulsifying wax and water. Alternatively, they can be formulated as a suitable lotion or cream, suspended or dissolved in, for example, a mixture of one or more of the following: mineral oil, sorbitan monostearate, a polyethylene glycol, liquid paraffin, polysorbate 60, cetyl esters wax, cetearyl alcohol, 2-octyldodecanol, benzyl alcohol and water.
[0153] Formulations suitable for topical administration in the mouth include lozenges comprising the active ingredient in a flavoured basis, usually sucrose and acacia ortragacanth; pastilles comprising the active ingredient in an inert basis such as gelatin and glycerin, or sucrose and acacia; and mouth-washes comprising the active ingredient in a suitable liquid carrier.
[0154] Generally, in humans, oral or topical administration of the compounds of the invention is the preferred route, being the most convenient. In circumstances where the recipient suffers from a swallowing disorder or from impairment of drug absorption after oral administration, the drug may be administered parenterally, e.g. sublingually or buccally.
[0155] For veterinary use, a compound of the invention is administered as a suitably acceptable formulation in accordance with normal veterinary practice and the veterinary surgeon will determine the dosing regimen and route of administration, which will be most appropriate for a particular animal.
Claims 1. An in vitro method of inducing apoptosis in a target cell comprising the steps: a. providing one or more target cells displaying the cell surface antigen, ICAM-I; b. providing one or more binding molecules which selectively binds to cell surface ICAM-I and, on binding ICAM- I, induces apoptosis of the target cell; c. exposing the target cells of (a) to the binding molecules of (b) to induce apoptosis in the target cells, wherein the binding molecules are human antibody molecules, said antibody molecules having variable regions having the sequences of figure 10. 2. A binding molecule which selectively binds to cell surface ICAM-I and, on binding ICAM-I, induces apoptosis of a target cell, wherein the binding molecule is a human antibody molecule, said antibody molecule having variable regions having the sequences of figure 10. 3. A binding molecule as claimed in claim 2 for use in the method of claim 1. 4. A binding molecule as claimed in either of claims 2 or 3 wherein the target cell is an immune cell or an epithelial cell. 5. A binding molecule as claimed in claim 4 wherein the immune cell is a B lymphocyte. 6. A binding molecule as claimed in any one of claims 2 to 5 wherein the target cell is associated with a disease. 7. A binding molecule as claimed in claim 6 wherein the disease is selected from the group consisting of: cancer: autoimmune diseases including but not restricted to rheumatoid arthritis and SLE, acute and chronic inflammatory disorders, sepsis and infectious disease including but not restricted to HIV. 8. A binding molecule as claimed in claim 7 wherein the disease is a cancer selected from lymphoma (leukemia, myeloma), gastric cancer, breast cancer, liver cancer, lung cancer, melanoma, bladder cancer, choroid cancer, pancreatic cancer, colon cancer and prostate cancer. 9. The binding molecule as claimed in any one of claims 2 to 8 wherein the antibody molecule is an IgG. 10. The binding molecule as claimed in Claim 9 wherein the IgG is selected from the group of an IgG.,, lgG2, lgG3or lgG4. 11. A nucleic acid having a nucleotide sequence encoding an antibody molecule as claimed in any one of claims 2 to 10. 12. A nucleic acid as claimed in claim 11 having the nucleotide sequences of figure 10. 13. A binding molecule as defined in any one of Claims 2 to 10 for use in the diagnosis and/or treatment and/or prevention of a disease, the diagnosis and/or treatment and/or prevention requiring the destruction of a target cell. 14. Use of the binding molecule as defined in any one of Claims 2 to 10 in the manufacture of a medicament for the treatment and/or prevention of a disease the diagnosis and/or treatment and/or prevention requiring the destruction of a target cell. 15. The binding molecule for use according to claim 13 or use according to claim 14 wherein the disease to be treated is selected from the group consisting of: cancer; autoimmune diseases including but not restricted to rheumatoid arthritis and SLE, acute and chronic inflammatory disorders, sepsis and infectious disease including but not restricted to HIV. 16. The binding molecule for use or use according to Claim 15 wherein the disease to be treated is cancer selected from lymphoma (leukemia, myeloma), gastric cancer, breast cancer, liver cancer, lung cancer, melanoma, bladder cancer, choroid cancer, pancreatic cancer, colon cancer and prostate cancer. 17. The binding molecule for use or use according to any one of claims 13 to 16 wherein the binding molecule or antibody molecule is as defined in either claim 1,2 or 3 and the disease to be treated is a lymphoma as defined in claim 16. 18. A pharmaceutical composition comprising the binding molecule as defined in any one of claims 2 to 10 and a pharmaceutically-acceptable carrier, excipient or diluent. 19. A binding molecule, binding molecule for use, nucleic acid, use or pharmaceutical composition as defined in any of claims 2 to 18 wherein the binding molecule selectively binds to cell surface ICAM-1 and, on binding ICAM-1, induces apoptosis of a target cell in vitro.
Patentansprüche 1. In-vitro-Verfahren zum Induzieren von Apoptose in einer Zielzelle, umfassend die folgenden Schritte: a. Bereitstellen einer oder mehrerer Zielzellen, die das Zelloberflächenantigen ICAM-1 aufweisen; b. Bereitstellen eines oder mehrerer Bindemoleküle, die selektiv an Zelloberflächen-ICAM-1 binden und durch
Binden von ICAM-1 Apoptose der Zielzelle induzieren; c. Aussetzen der Zielzellen von (a) den Bindemolekülen von (b), um Apoptose in den Zielzellen zu induzieren, wobei die Bindemoleküle humane Antikörpermoleküle sind, wobei die Antikörpermoleküle variable Regionen mit den Sequenzen aus Figur 10 aufweisen. 2. Bindemolekül, das selektiv an Zelloberflächen-ICAM-1 bindet und durch Binden von ICAM-1 Apoptose einer Zielzelle induziert, wobei das Bindemolekül ein humanes Antikörpermolekül ist, wobei das Antikörpermolekül variable Regionen mit den Sequenzen aus Figur 10 aufweist. 3. Bindemolekül nach Anspruch 2 zur Verwendung im Verfahren nach Anspruch 1. 4. Bindemolekül nach einem der Ansprüche 2 oder 3, wobei die Zielzelle eine Immunzelle oder eine Epithelzelle ist. 5. Bindemolekül nach Anspruch 4, wobei die Immunzelle ein B-Lymphozyt ist. 6. Bindemolekül nach einem der Ansprüche 2 bis 5, wobei die Zielzelle mit einer Krankheit verbunden ist. 7. Bindemolekül nach Anspruch 6, wobei die Krankheit ausgewählt ist aus der Gruppe bestehend aus: Krebs, Autoim-munerkrankungen, einschließlich aber nicht beschränkt auf rheumatoide Arthritis und SLE, akuten und chronischen Entzündungskrankheiten, Sepsis und Infektionskrankheiten, einschließlich aber nicht beschränkt auf HIV. 8. Bindemolekül nach Anspruch 7, wobei die Krankheit ein Krebs ist, ausgewählt aus Lymphom (Leukämie, Myelom), Magenkrebs, Brustkrebs, Leberkrebs, Lungenkrebs, Melanom, Blasenkrebs, Aderhautkrebs, Bauchspeicheldrüsenkrebs, Darmkrebs oder Prostata krebs. 9. Bindemolekül nach einem der Ansprüche 2 bis 8, wobei das Antikörpermolekül ein IgG ist. 10. Bindemolekül nach Anspruch 9, wobei das IgG ausgewählt ist aus der Gruppe von einem IgG^ lgG2, lgG3oder lgG4. 11. Nukleinsäure mit einer Nukleotidsequenz, die für ein Antikörpermolekül nach einem der Ansprüche 2 bis 10 codiert. 12. Nukleinsäure nach Anspruch 11 mit den Nukleotidsequenzen aus Figur 10. 13. Bindemolekül nach einem der Ansprüche 2 bis 10 zur Verwendung beim Diagnostizieren und/oder Behandeln und/oder Vorbeugen einer Krankheit, wobei das Diagnostizieren und/oder das Behandeln und/oder das Vorbeugen das Zerstören einer Zielzelle erfordern. 14. Verwendung des Bindemoleküls nach einem der Ansprüche 2 bis 10 in der Herstellung eines Medikaments zum Behandeln und/oder Vorbeugen einer Krankheit, wobei das Diagnostizieren und/oder das Behandeln und/oder das Vorbeugen das Zerstören einer Zielzelle erfordern. 15. Bindemolekül zur Verwendung nach Anspruch 13 oder zur Verwendung nach Anspruch 14, wobei die zu behandelnde Krankheit ausgewählt ist aus der Gruppe bestehend aus: Krebs, Autoimmunerkrankungen, einschließlich aber nicht beschränkt auf rheumatoide Arthritis und SLE, akuten und chronischen Entzündungskrankheiten, Sepsis und Infektionskrankheiten, einschließlich aber nicht beschränkt auf HIV. 16. Bindemolekül zur Verwendung oder Verwendung nach Anspruch 15, wobei die zu behandelnde Krankheit ausgewählt ist aus Lymphom (Leukämie, Myelom), Magenkrebs, Brustkrebs, Leberkrebs, Lungenkrebs, Melanom, Blasenkrebs, Aderhautkrebs, Bauchspeicheldrüsenkrebs, Darmkrebs oder Prostatakrebs. 17. Bindemolekül zur Verwendung oder Verwendung nach einem der Ansprüche 13 bis 16, wobei das Bindemolekül oder Antikörpermolekül nach einem der Ansprüche 1, 2 oder 3 definiert ist und die zu behandelnde Krankheit ein Lymphom nach Anspruch 16 ist. 18. Pharmazeutische Zusammensetzung, umfassend das Bindemolekül nach einem der Ansprüche 2 bis 10 und einen pharmazeutisch unbedenklichen Trägerstoff, Hilfsstoff oder Verdünner. 19. Bindemolekül, Bindemolekül zur Verwendung, Nukleinsäure, Verwendung oder pharmazeutische Zusammensetzung nach einem der Ansprüche 2 bis 18, wobei das Bindemolekül selektiv an Zelloberflächen-ICAM-1 bindet und durch Binden von ICAM-1 Apoptose einer Zielzelle in vitro induziert wird.
Revendications 1. Procédé in vitro d’induction de l’apoptose dans une cellule cible, comprenant les étapes consistant à : a. fournir une ou plusieurs cellules cibles présentant l’antigène de surface cellulaire, ICAM-I ; b. fournir une ou plusieurs molécules de liaison qui se lient de façon sélective à ICAM-I de surface cellulaire et, lors de la liaison à ICAM-I, induisent l’apoptose de la cellule cible ; c. exposer les cellules cibles de (a) aux molécules de liaisons de (b) pour induire l’apoptose dans les cellules cibles, dans lequel les molécules de liaison sont des molécules d’anticorps humain, lesdites molécules d’anticorps ayant des régions variables ayant les séquences de la figure 10. 2. Molécule de liaison qui se lie de façon sélective à ICAM-I de surface cellulaire et, lors de la liaison à ICAM-I, induit l’apoptose d’une cellule cible, laquelle molécule de liaison est une molécule d’anticorps humain, ladite molécule d’anticorps ayant des régions variables ayant les séquences de la figure 10. 3. Molécule de liaison selon la revendication 2, pour une utilisation dans le procédé selon la revendication 1. 4. Molécule de liaison selon l’une quelconque des revendications 2 ou 3, dans laquelle la cellule cible est une cellule immunitaire ou une cellule épithéliale. 5. Molécule de liaison selon la revendication 4, dans laquelle la cellule immunitaire est un lymphocyte B. 6. Molécule de liaison selon l’une quelconque des revendications 2 à 5, dans laquelle la cellule cible est associée à une maladie. 7. Molécule de liaison selon la revendication 6, dans laquelle la maladie est choisie dans le groupe constitué par : le cancer ; les maladies auto-immunes telles que, entre autres, la polyarthrite rhumatoïde et le lupus érythémateux disséminé (LED), les inflammations aiguës et chroniques, la sepsie et les maladies infectieuses telles que, entre autres, le VIH. 8. Molécule de liaison selon la revendication 7, dans laquelle la maladie est un cancer choisi parmi le lymphome (leucémie, myélome), le cancerde l’estomac, le cancerdu sein, le cancerdufoie, le cancerdu poumon, le mélanome, le cancerde la vessie, le cancerde la choroïde, le cancerdu pancréas, le cancerdu côlon et le cancerde la prostate. 9. Molécule de liaison selon l’une quelconque des revendications 2 à 8, dans laquelle la molécule d’anticorps est une IgG. 10. Molécule de liaison selon la revendication 9, dans laquelle l’IgG est choisie dans le groupe constitué par une IgG^ une lgG2, une lgG3 ou une lgG4. 11. Acide nucléique ayant une séquence nucléotidique codant pour une molécule d’anticorps selon l’une quelconque des revendications 2 à 10. 12. Acide nucléique selon la revendication 11, ayant les séquences nucléotidiques de la figure 10. 13. Molécule de liaison selon l’une quelconque des revendications 2 à 10, pour une utilisation dans le diagnostic et/ou le traitement et/ou la prévention d’une maladie, le diagnostic et/ou le traitement et/ou la prévention nécessitant la destruction d’une cellule cible. 14. Utilisation de la molécule de liaison selon l’une quelconque des revendications 2 à 10 dans la fabrication d’un médicament pour le traitement et/ou la prévention d’une maladie dont le diagnostic et/ou le traitement et/ou la prévention nécessitant la destruction d’une cellule cible. 15. Molécule de liaison pour une utilisation selon la revendication 13 ou utilisation selon la revendication 14, dans laquelle la maladie à traiter est choisie dans le groupe constitué par : le cancer ; les maladies auto-immunes telles que, entre autres, la polyarthrite rhumatoïde et le lupus érythémateux disséminé (LED), les inflammations aiguës et chroniques, la sepsie et les maladies infectieuses telles que, entre autres, le VIH. 16. Molécule de liaison pour une utilisation ou utilisation selon la revendication 15, dans laquelle la maladie à traiter est un cancer choisi parmi le lymphome (leucémie, myélome), le cancerde l’estomac, le cancerdu sein, le cancerdu foie, le cancer du poumon, le mélanome, le cancer de la vessie, le cancer de la choroïde, le cancer du pancréas, le cancer du côlon et le cancer de la prostate. 17. Molécule de liaison pour une utilisation ou utilisation selon l’une quelconque des revendications 13 à 16, dans laquelle la molécule de liaison ou la molécule d’anticorps est telle que définie selon la revendication 1,2 ou 3 et la maladie à traiter est un lymphome tel que défini dans la revendication 16. 18. Composition pharmaceutique comprenant la molécule de liaison selon l’une quelconque des revendications 2 à 10 et un vecteur, excipient ou diluant pharmaceutiquement acceptable. 19. Molécule de liaison, molécule de liaison pour une utilisation, acide nucléique, utilisation ou composition pharmaceutique selon l’une quelconque des revendications 2 à 18, la molécule de liaison se liant de façon sélective à ICAM-1 de surface cellulaire et, lors de liaison à ICAM-1, induisant l’apoptose d’une cellule cible in vitro.

Claims (2)

ÁpopóziM indlekáló ants-ICAM antitest Szabadalmi igénypontokOctopus Induction Ants-ICAM Antibodies Claims 1, M Vilm eljárás apopiozis indtAálására egy magában foglalja a 'S2fc&amp;$fógs$ lépéseket; 8$ rendelkezésre ^bocsátunk egy vagy több, ÍCAM4 seitíelüieti antigént bemutató eelsej-let: b) rendelkezésre hocsáfenk egy vagy több, se|ífelö!etl |CÁM~í~héZ: szelsktíveii kötődő kö-tőmolefeuiái amely(ek) az iCAM-ilyfeez Äldve a cél sej t apoptózisát indukálják; c) az (a) lépés szedntieéls^teket a (bj lépés szerinti kötőméiekulák: hatásának; tesszük ki, hogy a célsejtekben afmpőztst indukáljanak, ahol a kötőmokkidák humán antitest-molekulák, amelyek a IÖ. ábrán, bemutatott szekvenciákkal rendelkező variábilis régiókat tartalmaznak, % KMtaokteis, amely szeleMvert kitödlk a seltíélülei I€;AM-I~kez, és amely az 1€AM-I*hez torién© kötődés hatására egy célsejt apoptózisát indukálja, ahol a kőtőmolekula egy humán antitest-molekula, amely a 10. ábrán bemutatott szekvenciákkal rendelkező variábilis régiókat tartalmaz, 3 . A 2. igénypont szerinti kötőmolekula az 1. igénypont szerinti eljárásban történő alkalmazásra. 4. A 2. vagy 3, igénypont szerinti köÄtölekuja, ahol a célsejt egy immnnsejt vagy egy epitélsejt 5. A4 igénypont szerinti kötőmolekula, ahol az iramunsejt egy B-limíbeita, 6. Ä 2-5. igénypontok bámtelytke szerinti kötómokknla, ahol a célsejt egy betegséggel Összeföggő célsejt. 1, A $> Igénypont szerinti kötőmolekula, ahol a hétepég a kivetkezők közül van kiválasztva: tik, autoimmun betegségek, beleértve* többek között a reumaszeri izületi gyttlláriást és az SLE-t, akta és krónikus gyulladásos betegségek, szepszis és fertőző betegségek, beleértse, többek között, a ΙΊΙΥ-et.1, M Vilm's method for inducing apoptosis involves one of the steps of 'S2fc &amp; $ phos; $ 8 is available to provide one or more pre-antigen antigen presentations of αCAM4: b) available at one or more of the following binding molecules of the binding agent: iCAM-like By inducing apoptosis of the target cell; c) step (a) is a sedative for the effect of the binder (step bj): to induce apoptosis in the target cells, wherein the binding cocides are human antibody molecules containing variable regions having the sequences shown in Figure I,% KMtaokteis, which is excreted by the myocytes of I €; AM-I, and which induces apoptosis of a target cell by the action of 1 € AM-I * toriene, where the stone molecule is a human antibody molecule shown in Figure 10. The binding molecule of claim 2, for use in the method of claim 1. The binding molecule of claim 2 or 3, wherein the target cell is an immune cell or an epithelial cell according to claim 5, a binding molecule. wherein the iramune cell is a B-limb, the binding cell according to claims 6 to 5, wherein the target cell is a disease Conjugating Target Cell 1, A $> A binding molecule according to claim, wherein the weekend is selected from the projectors: tik, autoimmune diseases, including * including rheumatoid arthritis and SLE, dos and chronic inflammatory diseases, sepsis and infectious diseases , include, among others, ΙΊΙΥ. 8. A Ί. igénypont szerinti kotomoleknla, ahol a betegség a következők közül kiválasztott rákbetegség: .emtöáfe, &amp;á|rák, tüdőrák, melanoma, Míyagrák, érhártyadaganaí, és pmsztatarák. 9. A 2-8. igénypontok bármelyike szerinti kötőmolekula, ahol az anbtesőmolekuia egy IgG. lö. A 9. igénypont szerinti kötörnoleimia, ahol m %ö n Mvetkezökböf Ilié csoportiéi van kiválasztva: Igö; , IgClj, íg% és IgG*. I I, Puklelnsav, mm\y a 2-10, igénypontok Moteélyike szerinti sotitestemolokolái kódoló sukteoudszekvenciáva! rendelkezik. .12. A 11, igénypont szerimi nnkleinsav. amely a 10. ábrán bemutatott oaklemidszekven-eiákkai : modellezik. 13. A 2-10. igénypontok bármelyike szerinti köiomolekola egy betegség diagnosztizálására és/vágy kezelésére és/mgy megeltzésére történő alkalmazásra, ainoly dtagnoszizálás :é$/vagy kezelés és/vagy megelőzés egy eélsejt elpusztítását igényli. 14. A 2-10. igénypontok bármelyike szerinti kötömoleknla alkalmazása egy betegség diagnosztizálására és/vagy kezeléséi és/vngy ntegelözésére szolgáló gyógyszer előállítására,: amely diagnosztizálás és/vagy lezéíés és/vagy meplőzés egy eélseft elgnsztttásii igényli 15. A 13, igénypont szedni: kotönioiekula az igényelt alkalmazóra vagy a 14. Igénypont szerinti alkalmazás, ahol a kezelni kívánt betegség a kővetkezőkből álló csoportból van kiválasztva: rák. autoimmun betegségéL beleértve, többek között, a reomaszerö ízületi gyulladást és :Ó ikiAppttt és krónikus gyulladásos betegségek, szép szí s és fertőző betegségek, beleértve, többek között, aJílíf-éti 16. A 15. Igénypont szerinti kötömolekula az igényeli alMmazasfa, ahol a kezeim kívánt betegség a következői közül kiválasztott rákos betegség: limloma (leukémia, mielóraa), gyomorrák, emlőrák, máírák, tödirák,: melanoma, hólyagok, érhártyadaganat, hamyálmirigyv rák, vastagbélrák és prosztatarák. 17. A 13-16. ^émpjMlí bármelyike kőtőmolekula m Igényelt alkalmazásra vagy alkalmam, ahol a kőíőmoleknla vagy aotltest-moleknla az !·>,. 2. -vagy 3 - Ipnyfomha® definiált molekula, és a kezelni kivárd betegség a 16. Igéoyixmthan definiált limíoma. IS. Gyé^3#25s«|·. amely iaAáinaz egy 2-lü. ígéayimmok bámaelpke szerinti kötömolekulát és egy győgyászaülag elfogadható hordozói, segédanyagot vagy düuenst. 19. A 2-18. igénypontok bármelyle szerinti kötőmolekula, kőtömolekuia az igényelt alkalmazásra, nukieinsav, alkalmazás vagy gyógyászati készítmény, ahol a kötőmolekola szelektíven kötődik, a ssgíMüleii IGAM-NheZi.: é$ az l€AM~l-hez kötődve m vitro egy célsejt apopozlsái indokába.8. A Ί. The disease molecule of claim 1, wherein the disease is selected from the group consisting of: cancer, cancer, lung cancer, melanoma, myocardial cancer, vascular adrenal gland, and squamous cell carcinoma. 9. The binding molecule of any one of claims 1 to 3, wherein the antifungal molecule is an IgG. horse. The binder set according to claim 9, wherein m% f ng f li li li é é é: va va va: é é é é é é é é é é é é é é é é é é é é , IgCl1, Ig% and IgG *. I I, Phyclonic Acid, mm s of the Seto Test Molecules according to Claims 2 to 10, is a secto sequence. It has. .12. As claimed in claim 11, it is an acid. Fig. 10 is a model of the octet sequencers illustrated in Fig. 10. 13. Referring to FIGS. The binding molecule of any one of claims 1 to 5 for use in the diagnosis and / or treatment of a disease and / or prophylaxis of a disease, or dtagnosis: and / or treatment and / or prevention requires the destruction of a progenitor cell. 14. Referring to FIGS. The use of a binding molecule according to any one of claims 1 to 5 for the manufacture of a medicament for diagnosing and / or treating and / or treating a disease, wherein diagnosis and / or sealing and / or deposition is required by a prophylaxis of a primordial fungus. Use according to claim, wherein the disease to be treated is selected from the group consisting of: cancer. autoimmune disease including, but is not limited to, rheumatoid arthritis and: ikippAppttt and chronic inflammatory diseases, beautiful color and infectious diseases, including, but not limited to, lipid 16. The binding molecule of claim 15, wherein the hands are desired disease is a cancer disease selected from the group consisting of: limloma (leukemia, myeloma), gastric cancer, breast cancer, liver cancer, mumps, melanoma, bladder, vascular tumor, hamley-gland cancer, colon cancer and prostate cancer. 17. References 13-16. j j j j í í í ő ő ő ő ula ula ula ula ula elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt elt j elt j elt elt elt elt elt elt elt elt elt elt elt elt elt elt 2. - or 3 - Ipnyfomha®-defined molecule, and the disease being treated is a limioma defined by 16. Igeoyixmthan. It IS. 3, w hich ^ # 25s "| ·. which is alpha-2a. a promising molecule according to the invention and a pharmaceutically acceptable carrier, excipient, or suppository. 19. Referring to Figs. A binding molecule according to any one of claims 1 to 4, a rock molecule for the claimed use, a nucleic acid, an application or a pharmaceutical composition, wherein the binding molecule selectively binds, binding to ssgImIle IGAM-NheZi: $ 1 to AM-1 in vitro for reasons of apoptosis of a target cell.
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